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大肠杆菌氨甲酰磷酸合成酶的体外合成:精氨酸阻遏物参与累积阻遏的证据。

In vitro synthesis of Escherichia coli carbamoylphosphate synthase: evidence for participation of the arginine repressor in cumulative repression.

作者信息

Lissens W, Cunin R, Kelker N, Glansdorff N, Piérard A

出版信息

J Bacteriol. 1980 Jan;141(1):58-66. doi: 10.1128/jb.141.1.58-66.1980.

Abstract

A deoxyribonucleic acid-directed in vitro system for the synthesis of Escherichia coli carbamoylphosphate synthase has been developed, and its properties have been studied. The system uses the deoxyribonucleic acid of a lambda phage carrying the car genes (lambdadcarAB) as template and mediates the synthesis of both subunits of the enzyme. This newly synthesized enzyme exhibits the properties of native carbamoylphosphate synthase. A study of the in vitro synthetic capacities of S-30 extracts from strains containing either a mutated or the wild-type allele of gene argR supports earlier suggestions, based on in vivo evidence, that the argR product is involved in cumulative repression of carbamoylphosphate synthase by arginine and the pyrimidines. Repression in vitro is as efficient as in vivo. In keeping with such observation it is shown that in vitro synthesis of carbamoylphosphate synthase is repressed by partially purified arginine repressor. Evidence was obtained which indicates that arginine repression of carbamoylphosphate synthase mainly operates at the level of transcription. This was based on the design of an in vitro transcription system for gene carA, the structural gene for the light subunit of carbamoylphosphate synthase. This system also allowed us to demonstrate that free arginine is the corepressor involved in carbamoylphosphate synthase repression. The present in vitro approaches, in addition to the information they have already provided, open new possibilities for further investigations on the mechanism of cumulative repression and, in particular, on the participation of pyrimidine end products in this regulatory mechanism.

摘要

已开发出一种用于合成大肠杆菌氨甲酰磷酸合酶的脱氧核糖核酸指导的体外系统,并对其性质进行了研究。该系统以携带car基因(λdcarAB)的λ噬菌体的脱氧核糖核酸为模板,介导该酶两个亚基的合成。这种新合成的酶具有天然氨甲酰磷酸合酶的性质。对含有基因argR的突变等位基因或野生型等位基因的菌株的S-30提取物的体外合成能力的研究支持了基于体内证据的早期推测,即argR产物参与精氨酸和嘧啶对氨甲酰磷酸合酶的累积阻遏。体外阻遏与体内一样有效。与此观察结果一致,表明氨甲酰磷酸合酶的体外合成受到部分纯化的精氨酸阻遏物的阻遏。获得的证据表明,氨甲酰磷酸合酶的精氨酸阻遏主要在转录水平起作用。这是基于为氨甲酰磷酸合酶轻亚基的结构基因carA设计的体外转录系统。该系统还使我们能够证明游离精氨酸是参与氨甲酰磷酸合酶阻遏的辅阻遏物。除了已经提供的信息外,目前的体外方法为进一步研究累积阻遏机制,特别是嘧啶终产物在这种调节机制中的参与,开辟了新的可能性。

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